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牛精囊主要分泌蛋白与牛精子的结合。

Binding of a major secretory protein from bull seminal vesicles to bovine spermatozoa.

作者信息

Aumüller G, Vesper M, Seitz J, Kemme M, Scheit K H

机构信息

Department of Anatomy and Cell Biology, Philipps University, Marburg, Federal Republic of Germany.

出版信息

Cell Tissue Res. 1988 May;252(2):377-84. doi: 10.1007/BF00214380.

Abstract

The seminal vesicles synthesize in an androgen-dependent manner a neutral protein of 13.5 kDa molecular weight that makes up about 40% of their secretion ("major protein"). An antiserum against this protein raised in rabbits was used to localize the antigen within the seminal vesicles. In addition to intraluminal secretion of the seminal vesicles and the ampulla of the vas deferens, ejaculated and ampullary spermatozoa revealed an intense immunoreaction, which was restricted to the neck region of the sperm head and the middle piece, while the principal piece of the tail as well as the sperm head were devoid of immunoreactive material. Comparison of spermatozoa taken from the tail of the epididymis with ampullary spermatozoa showed that about 90% of the latter, but only 10-20% of the former presented this distributional pattern of immunoreactive sites. Epididymal epithelium as well as calf seminal vesicle epithelium showed no immunoreactivity with major protein antiserum. Using a pre-embedding staining technique with gold-labeled primary or secondary antibodies, respectively, no immunostaining could be achieved at the ultrastructural level. Incubation experiments of epididymal spermatozoa in EGTA-containing solutions in the absence of calcium resulted in a gradual labilization and eventual loss of the plasma membrane of the sperm middle piece. After removal of (at least part of) the plasma membrane, bound major protein could be visualized immunohistochemically close to the mitochondria of the middle piece using a gold-labeled primary or secondary antibody. The acceptor site for major protein therefore seems to reside inside the plasma membrane of the sperm middle piece.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

精囊以雄激素依赖的方式合成一种分子量为13.5 kDa的中性蛋白,该蛋白约占其分泌物的40%(“主要蛋白”)。用在兔体内产生的针对该蛋白的抗血清来定位精囊内的抗原。除了精囊和输精管壶腹的腔内分泌物外,射出的和壶腹内的精子显示出强烈的免疫反应,该反应局限于精子头部的颈部区域和中段,而尾部的主段以及精子头部则没有免疫反应性物质。将取自附睾尾部的精子与壶腹内的精子进行比较,结果显示,后者约90%呈现这种免疫反应性位点的分布模式,而前者只有10 - 20%呈现这种模式。附睾上皮以及小牛精囊上皮与主要蛋白抗血清均无免疫反应。分别使用金标记的一抗或二抗的包埋前染色技术,在超微结构水平未实现免疫染色。在不含钙的含乙二醇双乙醚二胺四乙酸(EGTA)溶液中对附睾精子进行孵育实验,导致精子中段的质膜逐渐不稳定并最终丧失。去除(至少部分)质膜后,使用金标记的一抗或二抗通过免疫组织化学方法可在中段线粒体附近观察到结合的主要蛋白。因此,主要蛋白的受体位点似乎位于精子中段的质膜内。(摘要截短于250字)

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